Gene silencing, knockout and over-expression of a transcription factor ABORTED MICROSPORES (SlAMS) strongly affects pollen viability in tomato (Solanum lycopersicum)

Background The tomato (Solanum lycopersicum L.) is an economically valuable crop grown worldwide. Because the use of sterile males reduces the cost of F1 seed production, the innovation of male sterility is of great significance for tomato breeding. The ABORTED MICROSPORES gene (AMS), which encodes for a basic helix-loop-helix (bHLH) transcription factor, has been previously indicated as an essential gene for tapetum development in Arabidopsis and rice. To determine the function of the SlAMS gene (AMS gene from S. lycopersicum) and verify whether it is a potential candidate gene for generating the male sterility in tomato, we used virus-induced gene silencing (VIGS), CRISPR/Cas9-mediated genome editing and over-expression technology to transform tomato via Agrobacterium infection. Results Here, the full-length SlAMS gene with 1806 bp from S. lycopersicum (Accession No. MK591950.1) was cloned from pollen cDNA. The results of pollen grains staining showed that, the non-viable pollen proportions of SlAMS-silenced (75%), −knockouted (89%) and -overexpressed plants (60%) were significantly higher than the wild type plants (less than 10%; P < 0.01). In three cases, the morphology of non-viable pollen grains appeared tetragonal, circular, atrophic, shriveled, or otherwise abnormally shaped, while those of wild type appeared oval and plump. Furthermore, the qRT-PCR analysis indicated that SlAMS in anthers of SlAMS-silenced and -knockouted plants had remarkably lower expression than in that of wild type (P < 0.01), and yet it had higher expression in SlAMS-overexpressed plants (P < 0.01). Conclusion In this paper, Our research suggested alternative approaches to generating male sterility in tomato, among which CRISPR/Cas9-mediated editing of SlAMS implied the best performance. We also demonstrated that the downregulation and upregulation of SlAMS both affected the pollen formation and notably led to reduction of pollen viability, suggesting SlAMS might be essential for regulating pollen development in tomato. These findings may facilitate studies on clarifying the SlAMS-associated molecular regulatory mechanism of pollen development in tomato. Supplementary Information The online version contains supplementary material available at 10.1186/s12864-022-08549-x.


Introduction
The tomato (Solanum lycopersicum Mill.) is a valuable self-pollinating fruit crop that is cultivated globally [1]. The tomato is imminently suitable for genetic engineering and as a model plant due to its small genome [2,3]. As the use of sterile males may reduce the cost of F 1 hybrid seed production, male sterility has the widespread application value and great prospects in tomato breeding [4]. Thus, many researchers have attempted to develop and identify male-sterile tomato lines. At present, hybrid tomato seed production is dominated by artificial emasculation and pollination, which is time-consuming and labor-intensive. In addition, in existing male-sterile tomato lines, it is difficult to maintain pollen infertility and stamen degeneration to ensure complete sterility [5,6]. As functional male sterility in tomato is also greatly affected by environmental conditions, these sterile types are rarely used for the production of tomato hybrids. Previously, various genes associated with male sterility in tomatoes have been mapped to various chromosomes using morphological and molecular markers. Based on studies of the molecular mechanisms regulating anther and pollen development in Arabidopsis and rice, abortive-pollen male-sterile tomato mutants have been artificially produced by knocking out key regulating genes [7].
Tapetum is the inner layer of plant anther wall. During the growth and development of plant pollen, the programmed cell death of tapetum provides necessary nutrients for the development of microspores [8]. Delayed or early degradation of the tapetum may adversely affect pollen development, leading to male sterility. Molecular techniques have previously been used to discover and clone genes related to tapetum development in rice [9], Arabidopsis [10] and petunias [11]. In Arabidopsis, the genes and transcription factors regulating early tape-  [12][13][14], and the gene expressed in the later tapetum development were reported as TAPETAL DEVELOPMENT AND FUNCTION1 (TDF1), ABORTED MICROSPORES (AMS), MYELOBLASTOSIS103 (MYB103), and MALE STERILITY1 (MS1) [15,16]. For example, mutations of SPL/NZZ led to development failures in the tapetum, as well as the pollen sac and spore mother cell primordium [17]. The transcription factors, DYSFUNCTIONAL TAPETUM1 (DYT1), TDF1, AMS, MS188, and MS1 form a pathway that controls tapetum development [18,19]. For example, DYT1, the most upstream regulator of tapetum development, affects many downstream genes associated with tapetum development and pollen wall formation by directly regulating TDF1 [20].
The AMS gene encodes a basic helix-loop-helix-like (bHLH) transcription factor. It has been reported that AMS and its direct downstream regulator MS188 are essential for tapetum development: AMS mutants developed abnormally enlarged tapetum cells and abortive microspores in Arabidopsis [21,22]. In addition, the AMS protein combines with MS188 (or other MYB proteins) and bHLH010 (or other bHLH proteins) to regulate the expression of the sporopollenin synthesis gene [23]. AMS regulates the temporal and spatial expression of 23 genes, such as CYTOCHROME 703A2 (CYP703A2), POLYKE-TIDE SYNTHASE A/B (PKSA/PKSB), TETRAKETIDEa-PYRONE REDUCTASE1 (TKPR1) and CYP704B1, precisely controlling several important life processes associated with pollen wall formation, including enamel and primary wall synthesis, as well as sporopollenin synthesis, transport, and deposition. AMS also affects microspore development, participates in the control of anther cell differentiation, and plays a role in biphasic regulation of tapetum development and pollen abortion in Arabidopsis [24,25].
The AMS gene has been identified and characterized in several plants besides Arabidopsis. For example, in Capsicum annuum L., CaAMS was preferentially expressed in the tapetum during the tetrad and earlyintermediate mononuclear stages; CaAMS downregulation led to the partial shortening of the capsicum flower, atrophy, unbroken stamens, and aborted pollen. By contrast, in CaAMS-silenced anthers, several genes involved in the formation of the outer pollen walls were downregulated [26]. Similarly, rice TAPE-TUM DEGENERATION RETARDATION (TDR), which was shown to be orthologous to Arabidopsis AMS, is preferentially expressed in the tapetum and encodes a putative bHLH protein; in rice, TDR is a key component gene of the molecular network regulating tapetum development and degeneration [16,27]. Finally, it was shown that the silencing of the AMS homolog in melon (Cucumis melo L.) led to male sterility [4]. Thus, AMS may represent a candidate gene for the control of male sterility.
In this study, we aimed to determine whether SlAMS was a potential candidate gene for the development of male-sterile tomato lines. First, we cloned the tomato SlAMS gene using reverse transcription-polymerase chain reactions (RT-PCR), and predicted the physicochemical properties and structural characteristics of the AMS protein. Second, we verified SlAMS function using virus induced gene silencing (VIGS). Finally, we constructed an SlAMS knockout vector using the CRISPR/Cas9-mediated genome editing system, and an SlAMS overexpression vector using plasmid pCAMBIA2301. We then assessed the viability and morphology of the pollen grains produced by untransformed plants carrying either the SlAMS silencing, knockout, or overexpression vector. Our research might not only create the new male sterility materials which would be able to be used in tomato breeding, but also be significant for the further deeply understanding the mechanism of pollen development and regulation in tomato.

Characterization of the tomato AMS gene
The tomato SlAMS gene was successfully cloned. The amplified fragment was about 1.8 kb long (Fig. 1a); six single colonies were verified using PCR (Fig. 1b). The full length of the tomato SlAMS gene was 1806 bp, which contained the complete open reading frame (ORF) region (Additional file 1). The cloned SlAMS sequence was submitted to GenBank (Accession No. MK591950.1). Nucleotide similarity analysis of SlAMS gene sequences indicated that the identity percentage of the cloned SlAMS gene varied from 78 to 100% when compared with the known sequences (Additional file 12), and the Solanaceae crops shared the higher sequence similarity (85% ~ 100%) as well.
The phylogenetic analysis showed that the tomato SlAMS protein (GenBank ID: QDO73362.1) formed a larger, well-supported Solanaceae clade that included S. pennellii (XP_027774838.1), S. tuberosum (XP_0063515 93.1), Capsicum annuum (XP_016537577.1), hysalis pubescens (AZB50351.1) and Nicotiana attenuata (OIT32810.1; Fig. 2). The phylogenetic tree also identified genetic evolution relationship of AMS proteins in other economically important crops, such as C. annuum, Helianthus annuus (XP_022028120.1), Brassica napus (XP_022562176.1), Raphanus sativus (XP_018437312.1), and Glycine max (XP_025979976.1). Our phylogenetic tree indicated a close evolutionary relationship among the tomato SlAMS protein and other Solanaceae plants, suggesting that it may be generally conserved within The predicted tomato SlAMS protein contained 602 amino acid residues: serine (S) was the most abundant residue (9.3%), followed by leucine (E; 7.6%) and arginine (R; 5.5%; Fig. 3a). The protein included 89 negative charges (Asp + Glu) and 64 positive charges (Arg + Lys). Subcellular localization analysis predicted that the tomato SlAMS protein would be confined to the nucleus (Fig. 3b). The putative secondary structure of the protein was comprised of 16.64% α-helixes, 70.04% random coils, and 10.32% extended chains ( Fig. 3c and Additional file 2). Consistent with the secondary structure prediction, the predicted tertiary structure of the tomato SlAMS protein was generally ellipsoidal, and primarily composed of random coils (Fig. 3d). of SlAMS-silenced plants (75%) were extremely significantly higher than that of the wild type and negative control plants (P < 0.01; Fig. 4c), Pollen grains staining results also showed that the pTRV2 virus carrier had little effect on pollen activity. After SlAMS gene silencing, the activity of the tomato pollen decreased significantly. Under the SEM, the pollen grains from the SlAMS-silencing plants appeared irregular shape (tetragonal, sunken and shriveled), while the wild type plants performed oval and plump (Fig. 4d, WT).

Pollen viability and morphology of SlAMS-knockouted plants
After the successful construction of the knockout vector CRISPR/Cas9-SlAMS confirmed by sequencing, tomato genetic transformation was performed using Agrobacterium-mediated methods. The transformation procedure using cotyledon as explants included pre-culture, Agrobacterium infection, co-culture, selection culture, regenerating and rooting culture. In total, 38 regenerated plants were obtained using selection medium supplemented with kanamycin. Among them, 33 plants were identified as positively transformed via the PCR identification of the kana-resistance gene Npt II (Fig. 5a).
To identify mutations of SlAMS gene in these positively transformed plants, we conducted sequencing of amplification products of the SlAMS fragments, the results indicated that 21 mutant out of 33 Npt II positive plants were identified as mutants, thus the frequency of mutations was about 63.6%. The types of SlAMS editing in mutant plant were almost single base mutation, including the 16th base A of target sequence mutated to G, the 15th base T to C, and 14th base C to A (Fig. 5d). Previously study reported that the frequency deletion correlated with the target site in tomato via CRISPR/Cas9 system, the ratio of 1 to 10 bp deletion was about 67%, but only 3% for 10 bp or higher deletion [28]. It was obvious that shorter deletions such as 1 bp appeared at high frequency in our system.

SlAMSsilencing
Negative control Despite the SlAMS-knockout plants blossomed normally in anthesis ( Fig. 4a; Additional file 5 Fig. S5c), the pollen grains were poorly developed, and about 89% pollen grains were stained blue (Fig. 5b, SlAMS-knockout). This indicated that only 11% of the grains were viable. In the untransformed wild type plants, pollen viability proportion was 92% (Fig. 5b, WT). The percentage of nonviable pollen grains of SlAMS knockout plants (89%) were extremely significant higher than that of the wild type plants (P < 0.01; Fig. 4c). Under the SEM, the pollen grains from the SlAMS-knockout plants appeared round, diamond-like or shrinkage ( Fig. 4d; Fig. 5c, SlAMSknockout). In contrast, pollen grains from the wild type plants appeared oval ( Fig. 4d; Fig. 5c). Thus, both pollen staining and SEM observation indicated that SlAMS knockout remarkably reduced pollen viability as compared to the wild type plants.

Pollen viability and morphology of SlAMS-overexpressed plants
PCR verification of the positive colonies indicated that the target amplicon was about 1800 bp in length (Additional file 6). After implementing Agrobacteriummediated transformation (Additional file 7), PCR detection of the Npt II gene showed that 17 plants had been successfully transformed with pCAMBIA 2301-SlAMS (Additional file 8).
The characters at florescence stage in the SlAMSoverexpressed plants were shown in Fig. 4a and Additional file 5 Fig. S5d. In viability test, pollen grains were poorly developed, and about 60% were stained blue. This indicated that merely 40% of the pollen grains were viable, while the proportion in wild type plants were 91% (Fig. 5b). The ratio of non-viable pollen grains of SlAMSoverexpressed plants (60%) were notably higher than that  Fig. 4c). Under the SEM, the pollen grains from the SlAMS-overexpressed plants were rhombic, atrophic, shriveled, or otherwise abnormally shaped ( Fig. 4d; Fig. 5c). Thus, both pollen staining and SEM observation indicated that SlAMS overexpression considerably reduced pollen viability as compared to the wild type plants. See Additional file 16 for all unedited gel pictures in the paper.

qRT-PCR analyses of SlAMS
We performed qRT-PCR using RNA from SlAMSsilenced, −knockouted, −overexpressed anthers to verify whether those biotechnological system would be effective, and further if the down or upregulation of SlAMS affect pollen development in tomato. The qRT-PCR analysis showed that, both at tetrad and maturity stage, the expression levels of SlAMS in silencing and knockout anthers reduced significantly (P < 0.01) when compared with that of wild type anthers (Fig. 6), thus demonstrated that the SlAMS expressions were downregulated after being silenced and knockouted (SlAMS-knockout plants conferred the lower expression level), and as a result, the abnormal pollen development occurred and abortive pollen produced in those plants. But noticeably, the qRT-PCR results appeared SlAMS had higher expression in overexpressed anthers contrasted to in that of wild type anthers (P < 0.01), the upregulation of SlAMS also affected the pollen formation and led to the decreasing of viability. Combined the results of qRT-PCR, pollen viability and morphology assessments, the compound results suggested that SlAMS might be essential for regulating pollen development in tomato.

Discussion
Although pollen development is an extraordinarily complicated process, several transcription factors that regulate tapetum development have been cloned and their function identified, including DYT1, TDF1, AMS and MS188 [18,20,22,29]. Here, we cloned a candidate tomato gene, SlAMS (1806 bp), which may be essential for tapetum and pollen development and result in male sterility in tomato. Our phylogenetic tree indicated a close evolutionary relationship among the SlAMS proteins and other plants, suggesting that SlAMS may be generally conserved within families, especially conserved across this group of the Solanaceae (e.g., S. pennellii, potato, and pepper). The SlAMS protein was also located in the nucleus and was primarily composed of irregular curls, implying that SlAMS acts as a transcription factor, regulating the expression of nuclear genes. The cloned CaAMS from Capsicum annuum also encodes a bHLH transcription factor and is localized to the nucleus, it seems to play an crucial role in pollen and tapetum development in pepper by regulating a complex network [26]. Due to the emasculation procedure of manual removing anthers, the costs of F1 seed production will be raised in major horticultural crops such as tomato and pepper, however, the utilization of male sterility is a very effective approach to solve the hybrid seed costs problem and ensure the high purity. Tomato male sterility has been an interest for current researchers. To date, the application of male sterility in cross breeding of tomato has not been successfully carried out for the mutants are nearly spontaneous, which requires a long period to eliminate linkage drags in backcrossing process. Besides the reported male-sterile mutants of MS32 and MS10 35 [30,31], recent researchers have demonstrated that male sterility in tomato plant was acquired after modifying of the SlMS10 gene via CRISPR/Cas9-mediated system, which could be introduced into the elite lines [28]. It was considered that the SlMS10 and MS32 were the upstream genes of AMS-like genes involved in pollen and tapetum development, the loss function of these genes resulted in downregulation of the other transcription factors gene such as AtTDF1-like, AtAMS-like, AtMYB-like and AtMS1-like in tomato [28,31]. Similarly, the downregulation of the CaAMS gene by VIGS system also led to male sterility in pepper and melon [26]. In this study, we demonstrated that alternative approaches to generating male sterility in tomato crop by the gene silencing, −knockout and -overexpression of the SlAMS gene, of which CRISPR/ Cas9-mediated genome editing of SlAMS conducted the best performance with the lowest viable pollen ratio (11%). Recently Jung et al. reported that the T1 and T2 generations of elite male-sterile lines, exhibiting abnormal tapetum and producing no pollen, were obtained by knockout of SlMS10 in tomato [28]. In comparison with the previously work, although we have obtained the pollen abortion-type male-sterile material in tomato, more research work must be conducted in the future. Firstly, as we used variety ' Ailsa Craig' in which was successfully established the highly effective genetic transformed system, it is necessary but time-consuming to eliminate linkage drags by executing backcross breeding process to transfer the male sterility trait to the comprehensive parents, moreover further transformation investigation would be done in the elite inbred lines so as to performing CRISPR/Cas9-mediated gene knockout. Secondly, We expected that the SlAMS-knochouted plants would have the most valuable application prospects for the highest proportion of non-viable pollen. Nevertheless, pollens of the knockout plants were not entirely abortive, 11% pollens still fertile. This may lead to pseudohybrids if utilized in hybrid seed production, hence the CRISPR/ Cas9-mediated system should be optimized such as editing site selection, and the hybrid process should be done to assess the practical application value and prospects in hybrid breeding in tomato.
It was clearly reported that two conserved pathway, namely, the DYT1-TDF1-AMS-bHLH10/89/91-MYB80 transcription cascade in Arabidopsis and the UDT1-TDR1-TIP2-EAT1 in rice [31,32]. With regard to the AMS gene, it has been cloned in Arabidopsis and other model plants, and the mechanisms by which AMS controls anther development in Arabidopsis have been well studied [16]. Indeed, previous studies have demonstrated that AMS plays a central role in the coordination of sporopollenin biosynthesis and the secretion of materials for pollen wall patterning [33], and the AMSlike gene is requried for anther and microspore development in pepper [26]. However, the role of the SlAMS gene in the regulatory network controlling pollen and tapetum development in tomato has not yet been investigated so far. Ferguson et al. reported that, in Arabidopsis, the biphasis expression was essential for tapetum and pollen formation, along with an initial peak around pollen meiosis and then later during pollen wall development, and AMS protein may competitively form a protein complex with other transcription factors, causing the repression of upstream regulators and promotion protein degradation, the researchers also indicated that additional factors are associated with the AMS regulation [24]. Noticeably, in this paper, the over-expression of SlAMS gave rise to the upregulation of SlAMS both at tetrad and maturity stages, and thus affected pollen formation and led to the decreasing of pollen activity in tomato plants. We deduced that the SlAMS upregulation might competitively repress the expression of upstream transcription factors such as MS, DYT1 or TDF1. It was indicated in our study that the gene silencing, knockout and over-expression of the tomato SlAMS gene strongly affected the its expression levels, and subsequently resulted in the morphological deformation of the pollen grains and pollen viability reduction, it is likely that AMS plays a crucial role in tapetal cell development and the post-meiotic transcriptional regulation of microspore development within the developing anther [16]. However, the expressions of other involved genes should be examined by qRT-PCR or RNA-seq in SlAMS-upregulated and downregulated plants to confirm the underlying pathway regulating the pollen and tapetum development.
In summary, in this paper, we only cloned the tomato SlAMS gene and explored the possibility of creation the novel male-sterile materials in tomato by SlAMS gene silencing, knockout and overexpression technology. Our results have laid a fundamental foundation for follow-up studies investigating the SlAMS-associated molecular mechanism regulating anther formation in tomatoes, as well as the creation of male-sterile tomato lines. Up to now, we have being carried out the further research work and made some progress: the pollen viability is measured in T1 progeny transgenic plants, having used the anther and pollen sample in different developmental stage to conduct transcriptome studies in SlAMS-knochouted and -overexpressed plants, we expect that the SlAMS-associated regulatory networks and pathways regulating pollen development and pollen fertility would be clarified in further studies.

Conclusion
To reduce the cost of hybrid seed production and ensure high purity, it is important to utilize the male sterility in crossbreeding of tomato. In this study, the SlAMS gene from tomato pollen cDNA was isolated and characterized. The sequencing results indicated that the tomato SlAMS gene had the length of 1806 bp encoding 602 amino acid residues. In addition, bioinformatics analysis showed that SlAMS gene shared the higher sequence similarity (85% ~ 98%) and exhibited a close evolutionary relationship with other known AMS in Solanaceae speices. Subsequently, by the use of VIGS, CRISPR/Cas9 and overexpression biotechnology, the proportion of non-viable pollen grains in SlAMS-silenced (75%), −knockouted (89%), and -overexpressed (60%) tomato plants were extremely significant higher than that of the untransformed plants (P < 0.01). The morphology performances in three cases of non-viable pollen grains comprised tetragonal, circular, atrophic, shriveled, or otherwise abnormally shaped, while pollen grains of the wild type plants appeared oval and plump. The qRT-PCR results indicated that the expression levels in anthers of SlAMSsilenced and -knockout plants were extremely lower than that of wild type plants, yet SlAMS gene had higher expression level in anthers of of SlAMS-overexpressed plants.
Thus, we demonstrated that the gene-silencing, − knockout and -overexpression of the SlAMS gene in tomatoes induced the SlAMS downregulation or upregulation, and this may lead to abnormal pollen development, which in turn decrease pollen viability, and subsequently generate male-sterile lines. Our research suggested alternative approaches to generating male sterility in tomato crop, among them, CRISPR/Cas9mediated genome editing of SlAMS implied the best performance.

Plant materials
Tomato (Solanum lycopersicum L.) plants of cv. ' Ailsa Craig' were grown in a greenhouse at Yunnan Agricultural University (Kunming, China). Greenhouse temperature was maintained at 26 °C during the day (16 h) and at 18 °C during the night (8 h). Tomato flower buds were removed from the plants at flowering period and placed in an ice box. Anthers were collected under low temperatures, quickly treated with liquid nitrogen and stored at − 80 °C.

Cloning and characterization of the tomato SlAMS gene
Total RNA was extracted from tomato anthers using Trizl Kits (TransGen Biotech. Co., Ltd., Beijing, China). The cDNA of the tomato was synthesized using High Fidelity Prime Script RT-PCR Kits (Takara Biomedical Technology Co., Ltd. Beijing, China), following the manufacturer's instructions, and amplified using PCR with the primers AMSad1 and AMSad2 (Additional file 13). Primers were designed based on the previously-published tomato AMS gene sequence (GenBank ID. LOC101253608) using Primer 5.0. The PCR volume contained 2 μL cDNA, 1 μL each primer (10 μmol/μL), 12.5 μL of 2 × EasyTaq PCR SuperMix, and ddH 2 O to make 25 μL. The PCR cycling conditions were as follows: pre-denaturation at 95 °C for 3 min; 35 cycles of denaturation at 94 °C for 50 s, annealing at 50 °C for 1 min, and extension at 72 °C for 3 min; a final extension at 72 °C for 10 min; and an indefinite hold at 4 °C. The target DNA fragment was extracted from the agarose gel using by gel filtration, and the purified using a TIANgen Midi Purification Kit (TIANGEN Biotech. Co., Ltd., Beijing, China) following the manufacturer's instructions. The target fragment was ligated to the pMDT-18 cloning vector (0.5 μL of vector, 4 μL of PCR product, 5 μL of Solution I, and 0.5 μL of T4 DNA ligase) to form pMDT-18-SlAMS, incubated at 16 °C for 3 h, and then transformed into Escherichia coli DH 5α competent cells. The transformed cells were cultured overnight at 37 °C. Six single white colonies were selected, and the length of the inserted fragment was confirmed using PCR. Recombinant plasmid DNA was isolated using TIANprep Mini Plasmid Kits (Yunnan Morning Green Biotechnology Co., Ltd. Yunnan, China) and sequenced by the Shuo Qing Biotechnology Co., Ltd. (Kunming, China).
The homology of the cloned SlAMS gene sequence was investigated using DNAMAN 6.0 and NCBI BLAST. To compare the predicted tomato SlAMS protein with other AMS homologs, both within the Solanaceae and among other closely-related families (i.e., the Compositae, Cruciferous, Leguminosae, and Cucurbitaceae), we constructed a phylogeny of the AMS proteins from 25 plant species (Additional file 14) using the neighbor-joining method in MEGAX10.1.5. A subcellular localization analysis was performed using PSORT II predict. The primary structure of the encoded SlAMS protein was predicted using PredictProte; the secondary structure was predicted using SOPMA; and the tertiary structure was predicted using SWISS-MODEL. The websites for the online tools are given in Additional file 15.

Obtaining the SlAMS-silenced plants by VIGS and morphological observation of pollen
We designed the primers AMS-F and AMS-R (Additional file 13) to amplify the SlAMS-interference fragment which was 274 bp long (Additional file 1), using the SNG VIGS TOOL (https:// vigs. solge nomics. net/) and pTRV2 as a basic VIGS vector (Additional file 9), we amplified the interference fragment from cloning vector pMDT-18-SlAMS as a template. We chose tobacco brittle virus (TRV) as gene silencing vector [34,35]. The TRV genome contains two RNA chains, RNA1 and RNA2, which form binary vectors. TRV vector-mediated gene silencing requires the simultaneous action of the RNA1 and RNA2 chains [36]. The pTRV2 vector was doubledigested with Sac I and Bam HI, and then ligated to the SlAMS-interference fragment to form the pTRV2-SlAMS carrier. The recombinant SlAMS products were then transformed into E. coli DH 5α and Agrobacterium tumefaciens GV310. SlAMS clones were verified using colony PCR with the primers AMS-R and pTRV2-seqE (Additional file 13) and then sequenced. The positive clones were fully mixed with 50% glycerin (a glycerin: bacterial culture ratio of 1:1) and stored at − 80 °C.
Tomato plants were randomly selected and allocated among four groups: plants in the silencing group were infected with A. tumefaciens carrying pTRV2-SlAMS and pTRV1; plants in the albefaction group (mock-infection) were infected with A. tumefaciens carrying pTRV2-PDS and pTRV1; plants in the negative control group were infected with A. tumefaciens carrying pTRV2 and pTRV1; and plants in the blank control group were uninfected wild type plants. Each group was represented by three replicates, and each replicate was comprised of 10 plants.
To activate Agrobacterium, 20 μL of glycerol-stored Agrobacterium carrying pTRV2-SlAMS, pTRV1, pTRV2, or pTRV2-PDS were added to 1 ml of Luria-Bertani medium (supplemented with 50 μg/ml kanamycin and 25 μg/ml rifampicin), and incubated overnight at 28 °C with shaking at 200 rpm. After incubation, the bacterial solution was added to 10 ml of LB medium and cultured overnight at 28 °C with shaking at 200 rpm. The bacterial solution was then centrifuged at 800 g for 15 min. Each A. tumefaciens pellet was resuspended in sufficient infection solution to make an optical density (OD) at 600 nm of 1.0. Then, each A. tumefaciens solution (carrying pTRV2-SlAMS, pTRV2, or pTRV2-PDS) was separately mixed with pTRV1 at a volume ratio of 1:1. The A. tumefaciens mixtures were cultured at 28 °C with shaking at 50 rpm for 3 h. After two euphyllas had completely unfolded, 30 plants per group were injected with 1 ml of the appropriate A. tumefaciens solution; the plants in the blank control group were injected with sterile water. After injection, plants were incubated in the dark at 21 °C for 24 h, and then cultivated in the greenhouse, covered with nylon nets to avoid cross-contamination and insectmediated virus transfer, until flowering.
Pollen was collected from five flowers from each plant in the wild type, negative control, and SlAMS-silenced groups. Pollen viability was measured using the blue-ink staining method. In brief, a small amount of pollen was placed on a glass slide, and a drop of distilled water was added. The pollen grains were spread out with tweezers, and then a drop of blue ink solution was added. Viable and non-viable pollen grains were counted in three different fields of view, and the final percent viable was calculated as the average of the three counts; unstained pollen were viable, while blue-stained pollen were abortive. The significance analysis of non-viability pollen percentage was implemented using t test method by statistical software SPSS 25.0. The morphological characters of the pollen grains were then observed under a scanning electron microscope (SEM) with an acceleration voltage (EHT) of 3.0 kv and a magnification (MAG) of 1.2 k.

pCRISPR/Cas 9-mediated SlAMS knockout and mutation analysis
A pCRISPR-SlAMS vector was constructed using a Cas9/ gRNA plasmid construction kit (VK005-08, Beijing Viewsolid Biotech., Co., Ltd., Beijing, China), following the manufacturer's instructions. In brief, the target gRNA sequence was designed based on the cloned SlAMS gene sequence using an online CRISPR design tool (crisPr. mit. edu). We then designed sense and anti-sense primers (pCRISPR-Sens and pCRISPR-Anti, respectively; Additional file 13) based on the target sequence and synthesized the oligomer. The oligomer was inserted into the Cas9/gRNA vector and transformed into E. coli DH 5α (Additional file 10). Then, colonies were randomly selected and sequenced to identify positive clones using the primers pCRISPR-SeqE (Additional file 13). The identified pCRISPR-SlAMS vector was transformed into A. tumefaciens GV3101. Then, we used Agrobacteriummediated method to transform the vector into tomato genome [37]. We conducted three batches of Agrobacterium infection using cotyledons (i.e 3 replicates), which comprised 80 ~ 100 explants in each batch.
After the co-culture, selection culture of the infected cotyledons, the regenerated plants were obtained. The genomic DNA were extracted from T0 progeny regenerated plants using the CTAB method. Regenerated but untransformed plants were used as controls. We detected transgenic plants via the PCR amplification of the Npt II selection gene. The PCR volume included 1 μL DNA; 2 μL 10 × PCR buffer, 0.4 μL dNTP mixture (2 mmol/L each), 0.2 μL forward and reverse primers (10 μmol/L), 0.2 μL Taq DNA polymerase (1 U/μL); and ddH 2 O to make 20 μL. The thermal cycling procedure was as follows: 94 °C for 3 min; 30 cycles of denaturation at 94 °C for 30 s, annealing at 58 °C for 30 s, and extension at 72 °C for 30 s; and a final extension at 72 °C for 10 min. In the CRISPR/Cas9 system, the Cas cleavage site occurs mostly 3 bp upstream of the protospacer, thus the insertion and deletion mutations around 3 bp upstream of the protospacer were considered to be mutations induced by Cas9. To identify the mutations, we designed the primers (AMS-F2/AMS-R2, Additional file 13) based on the gene editing site of SlAMS, and extracted the flower DNA of 33 individual Npt II positive plants. DNA extraction and PCR cycling conditions were the same as the Npt II ampification. The 267 PCR products were sequenced and confirmed for mutation (ShuoQing Biotech., Co., Ltd., Kunming, China).
The positive transgenic plants and the untransformed wild type plants were then cultivated in the greenhouse until flowering (covered in a nylon net to avoid crosscontamination as above). Pollen viability ratios in the control and transgenic plants were assessed as described above. The methods of statistic analysis and morphological observation of pollen grains were conducted as described above.

Agrobacterium-mediated SlAMS overexpression
Primers 2301-AMSF and 2301-AMSR (Additional file 13) were designed to amplify the SlAMS gene, using clone vector pMDT-18-SlAMS as a template. The SlAMS target gene fragment was ligated to the pCAMBIA2301 vector after digestion with Sac I and Bam HI to construct the overexpression vector pCAMBIA2301-SlAMS (Additional file 11). The recombinant product was transformed into E. coli DH 5α and A. tumefaciens GV3101. After verification of a single colony using PCR and sequencing, the positive clones were fully mixed with 50% glycerin (a glycerin: bacterial culture ratio of 1:1) and stored at − 80 °C.
Agrobacterium-mediated transformation was performed using cotyledons as target infection explants as described above. Three batches of Agrobacterium infection using cotyledons were conducted. The transgenic plants were then cultivated until flowering as described above. The genomic DNA of T0 progeny transformed plants were extracted by CTAB method and then detected transgenic plants via the PCR amplification of the Npt II gene contained in the overexpression vector pCAMBIA2301. Pollen viability and morphology were compared among the positive transgenic plants and the control plants as described above. The methods of statistic analysis and morphological observation of pollen grains were the same as above.

Anther RNA extraction and qRT-PCR analyses of SlAMS
We collected the anthers of SlAMS-silenced, −knockouted, −overexpressed plants and wild type plants during the flowering period at two pollen formation stages (tetrad and maturity). Total RNA was isolated from anthers of two flower buds using Trizol Kits (TransGen Biotech. Co., Ltd., Beijing, China) following the manufacture's instructions, and the cDNA was synthesized via performing the reverse transcription as described in the cloning of SlAMS gene. For SlAMS gene expression level detection, the specific primers (qAMS-F/qAMS-R) for qRT-PCR were designed based on the cloned SlAMS. We used Actin (GQ337966.1) as the internal control gene for its stable expression level in different plant tissues (Actin-F/Actin-R). The primers used were listed in Additional file 13.
The qRT-PCR was conducted using TB Green ® Pri-meScript ™ RT-PCR Kit (TaKaRa Bio. Co., Beijing, China) following the manufacture protocol on ABI 7500 real-time PCR system (Applied Biosystems, USA). The 10 μL qRT-PCR volume contained 0.2 μL each primer (10 μL mol/μL), 5 μL of 2XTB Green RT-PCR Buffer, 1 μL cDNA (200 ng), 3.6 μL ddH 2 O. Cycling reaction conditions were 95 °C for 3 min, followed by 40 cycles of 10 s at 95 °C, 15 s at 60 °C, and 20 s at 72 °C. Three biological replicates (at least three plants for each replicate) were performed in qRT-PCR. The relative expression levels of SlAMS were calculated by the 2 −△△Ct method. The difference significant analysis was conducted via t test using statistic software SPSS 25.0.